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来自拟南芥的叶绿体天冬氨酸转氨酶:基因结构与蛋白质空间结构之间关系的研究。

Chloroplastic aspartate aminotransferase from Arabidopsis thaliana: an examination of the relationship between the structure of the gene and the spatial structure of the protein.

作者信息

Wilkie S E, Lambert R, Warren M J

机构信息

Department of Molecular Genetics, University College London, U.K.

出版信息

Biochem J. 1996 Nov 1;319 ( Pt 3)(Pt 3):969-76. doi: 10.1042/bj3190969.

Abstract

A clone encoding a plastid isoenzyme of aspartate amino-transferase (AAT5) was isolated from an Arabidopsis genomic library and its complete sequence determined. The gene for AAT5 (asp5) contains an open reading frame of 2447 bp comprising 11 exons separated by introns ranging in length from 74 to 207 bp. The upstream regulatory region contains a putative TATA box and multiple copies of two sequence motifs, CTCTT and AAAGAT, previously associated with nodule-specific gene activity in legumes. The deduced primary amino acid sequence of the protein product of asp5 was used to generate a three-dimensional structure of the AAT5 protein by using the computer program Sybyl: Biopolymer Composer and known AAT structures on the protein databases. Both the mature protein and its precursor protein containing a putative N-terminal transit peptide were modelled. The resulting structure of the precursor protein indicated that the transit peptide might also inhibit dimerization of the protein until after its translocation across the chloroplast membrane. The derived structure of the mature protein was then analysed in terms of its component elements of secondary structure, and the positions on the polypeptide back-bone corresponding to intron insertion sites were determined. It is observed that the introns tend to map to regions between structural subdomains of the protein and also map to sites on the surface of the molecule. The asp5 gene in Arabidopsis is thus consistent with Gilbert's exon-shuffling theory of gene evolution [Gilbert (1985) Science 228, 823-824]. A high degree of conservation of intron insertion sites between AAT genes from different plants and animals is observed, particularly within the part of the gene encoding a large beta-sheet structure that forms the structural and functional core of the protein. This beta-sheet structure is thus believed to compromise an ancient and very highly conserved moiety of the molecule.

摘要

从拟南芥基因组文库中分离出一个编码天冬氨酸氨基转移酶质体同工酶(AAT5)的克隆,并测定了其完整序列。AAT5(asp5)基因包含一个2447 bp的开放阅读框,由11个外显子组成,外显子之间被长度在74至207 bp之间的内含子隔开。上游调控区包含一个假定的TATA框以及两个序列基序CTCTT和AAAGAT的多个拷贝,这两个基序先前与豆科植物中的根瘤特异性基因活性相关。利用计算机程序Sybyl:Biopolymer Composer和蛋白质数据库中已知的AAT结构,使用asp5蛋白质产物的推导一级氨基酸序列生成了AAT5蛋白质的三维结构。对成熟蛋白及其含有假定N端转运肽的前体蛋白都进行了建模。前体蛋白的最终结构表明,转运肽可能也会抑制该蛋白的二聚化,直到其穿过叶绿体膜后才会解除抑制。然后根据成熟蛋白的二级结构组成元件对其推导结构进行分析,并确定多肽主链上与内含子插入位点相对应的位置。观察到内含子倾向于定位到蛋白质结构亚结构域之间的区域,也定位到分子表面的位点。因此,拟南芥中的asp5基因与吉尔伯特的基因进化外显子改组理论[吉尔伯特(1985年)《科学》228,823 - 824]相符。观察到来自不同动植物的AAT基因之间内含子插入位点具有高度保守性,特别是在编码形成蛋白质结构和功能核心的大β折叠结构的基因部分。因此,这种β折叠结构被认为是分子中一个古老且高度保守的部分。

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